Antigen-specific helper T-cell receptor genes

ABSTRACT

The present invention pertains to polynucleotides that encode CDR3 in TCR-[alpha] and TCR-[beta] chain genes of CD4+ helper T-cells that are specific to WT1 helper peptides having an amino acid sequence represented by SEQ ID NO: 123. The present invention further pertains to the peptides encoded by said polynucleotides. The present invention further pertains to CD4+ T cells into which TCR genes that contain said polynucleotides have been introduced, the induction of WT1-specific cytotoxic T-lymphocytes (CTLs) using the CD4+ T-cells, the treatment of cancer, etc.

This is a division of application Ser. No. 14/427,465, whose § 371(c) date is Mar. 11, 2015, which is a national stage of International Application No. PCT/JP2013/074748, filed Sep. 12, 2013, and claims priority to Japanese Patent Application No. 2012-200480, filed Sep. 12, 2012, all of which are incorporated herein by reference.

TECHNICAL FIELD

The present invention relates to polynucleotides contained in T cell receptor (TCR) genes of cancer antigen-specific helper T-cells. In particular, the present invention relates to polynucleotides encoding complementarity determining region 3 (CDR3) of each α-chain and β-chain of TCR of CD4⁺ helper T-cells specific to a WT1 helper peptide having an amino acid sequence shown in SEQ ID NO: 123. The present invention also relates to polypeptides encoded by these polynucleotides. Further, the present invention relates to CD4⁺ T-cells into which TCR genes containing these polynucleotides are introduced, induction and enhancement of WT1-specific cytotoxic T cells (WT1-specific CTL) using them, and treatment of cancers using them, and so on.

BACKGROUND ART

WT1 gene (Wilms' tumor 1 gene) is a gene which was identified as a gene responsible for Wilms tumor which is a renal cancer in children (Non-patent Documents 1 and 2). WT1 is a transcription factor having a zinc finger structure. Initially, WT1 gene was considered to be a tumor suppressor gene. However, subsequent studies (Non-patent Documents 3, 4, 5 and 6) showed that WT1 gene rather functions as an oncogene in hematopoietic tumors and solid cancers.

It was showed that peptide-specific cytotoxic T cells (CTLs) were induced by stimulating peripheral mononuclear cells in vitro using a WT1 peptide and that these CTLs damage tumor and cancer cells in hematopoietic tumors and solid cancers which express WT1 endogenously. Because CTL recognizes a WT1 peptide in a form of a complex in which the WT1 peptide is bound to a MHC class I molecule, such a WT1 peptide differs in accordance to MHC class I subtype (Patent Document 1, Non-Patent Document 7, Patent Documents 2, 3 and 4).

Existence of helper T cells specific to a cancer antigen is important for effective induction of CTL (Non-Patent Document 8). Helper cells are induced and activated by recognizing a complex of a MHC class II molecule and an antigen peptide on antigen-presentino cells. Activated helper T cells produce cytokines such as IL-2, IL-4, IL-5, IL-6, or interferons, and help proliferation, differentiation and maturation of B cells. Activated helper T cells also have a function to promote proliferation, differentiation and maturation of other subset of T cells (such as Tc cells). Thus, because activated helper T cells have a function to activate immune system by promoting proliferation and activation of B cells and T cells, it is considered that enhancing the function of helper T cells via a MHC class II binding antigen peptide (helper peptide) to enhance the effect of a cancer vaccine useful in cancer immunotherapy (Non-Patent Document 9).

Examples of helper peptides relating to WT1 which are presently recognized are a peptide binding to HLA-DRB1*04:01 molecule (Non-Patent Document 10), a peptide binding to HLA-DRB1*04:05 molecule, a peptide binding to HLA-DRB1*15:02 molecule (Patent Document 5), a peptide binding to HLA-DRB1*04:05 molecule, HIA-DRB1*15:02 molecule, HLA-DRB1*15:01 molecule, HLA-DPB1*09:01 molecule and HLA-DPB1*05:01 molecule (Patent Document 6).

However, sequences of T cell receptor (TCR) genes of antigen-specific CD4⁺ helper T-cells which recognize a helper peptide have not been known at all.

DOCUMENTS OF BACKGROUND ART Patent Documents

-   Patent Document 1: WO2003/106682 -   Patent Document 2: WO2005/095598 -   Patent Document 3: WO2007/097358 -   Patent Document 4: PCT/JP2007/074146 -   Patent Document 5: WO2005/045027 -   Patent Document 6: WO2008/105462

Non-Patent Documents

-   Non-Patent Document 1: Daniel A. Haber et al., Cell. 1990 Jun. 29;     61(7):1257-69. -   Non-Patent Document 2: Call K M et al., Cell. 1990 Feb. 9;     60(3):509-20. -   Non-Patent Document 3: Menke A L et al., Int Rev Cytol. 1998;     181:151-212. Review. -   Non-Patent Document 4: Yamaqami et al., Blood. 1996 Apr. 1;     87(7):2878-84. -   Non-Patent Document 5: Inoue K et al., Blood. 1998 Apr. 15;     91(8):2969-76. -   Non-Patent Document 6: Tsuboi A et al., Leuk Res. 1999 May;     23(5):499-505. -   Non-Patent Document 7: Oka Y et al., Immunogenetics. 2000 February;     51(2):99-107. -   Non-Patent Document 8: Gao F G et al., Cancer Res. 2002 Nov. 15;     62(22):6438-41. -   Non-Patent Document 9: Zeng G, J Immunother. 2001 May;     24(3):195-204. -   Non-Patent Document 10: Knights A J et al., Cancer Immunol     Immunother 2002 July; 51(5):271-81.

SUMMARY OF INVENTION Problem to be Solved by the Invention

Problems to be solved by the invention were to determine sequences of TCR genes of CD4⁺ helper T-cells specific to a WT1 helper peptide, to obtain CD4⁺ T-cells into which these ICR genes have been introduced, to enhance induction of WT1 specific CTL using such cells, and to treat or prevent cancers, and so on.

Means to Solve the Problem

The inventors studied vary hard to solve the above problems, and succeeded in isolating α-chain genes and β-chain genes of TCR of CD4⁺ helper T-cells specific to a WT1 helper peptide, and determined each CDR3 sequence. Further, the inventors introduced TCR genes containing the sequences thus determined into CD4⁺ T-cells, and succeeded in enhancing induction of WT1 specific CTL and damaging WT1 expressing cancer cells by use of the CD4⁺ T-cells. Thus, the inventors have completed the present invention.

That is, the present invention provides:

(1) A polynucleotide (referred as “αCDR3 polynucleotide”) having a nucleotide sequence selected from the group consisting of SEQ ID NOs: 1, 3, 5, 8, 10, 11, 13, 14, 16, 18, 20, 22, 23, 25, 27, 20, 30, 31, 33, 35, 37, 39, 41, 43, 45, 47, 49, 51, 53, 55, 56 and 58, wherein said polynucleotide encodes CDR3 of α-chain of TCR of a CD4⁺ helper T-cell specific to a WT1 helper peptide (WT1₃₃₂ peptide) having an amino acid sequence shown in SEQ ID NO: 123 or a variant sequence thereof. (2) A polynucleotide (referred as “βCDR3 polynucleotide”) a nucleotide sequence selected from the group consisting of SEQ ID NOs: 2, 4, 6, 7, 9, 12, 15, 17, 19, 21, 24, 26, 29, 32, 34, 36, 38, 40, 42, 44, 46, 48, 50, 52, 54, 57 and 59, wherein said polynucleotide encodes CDR3 of β-chain of TCR of a CD4⁺ helper T-cell specific to WT1₃₃₂ peptide. (3) A pair of a αCDR3 polynucleotide and a βCDR3 polynucleotide, wherein each polynucleotide has the following nucleotide sequence:

α CDR3 polynucleotide βCDR3 polynucleotide SEQ ID NO: 1 SEQ ID NO: 2 SEQ ID NO: 3 SEQ ID NO: 4 SEQ ID NO: 5 SEQ ID NO: 6 SEQ ID NO: 3 SEQ ID NO: 7 SEQ ID NO: 8 SEQ ID NO: 9 SEQ ID NO: 10 SEQ ID NO: 12 SEQ ID NO: 11 SEQ ID NO: 12 SEQ ID NO: 13 SEQ ID NO: 15 SEQ ID NO: 14 SEQ ID NO: 15 SEQ ID NO: 16 SEQ ID NO: 17 SEQ ID NO: 18 SEQ ID NO: 19 SEQ ID NO: 20 SEQ ID NO: 21 SEQ ID NO: 22 SEQ ID NO: 24 SEQ ID NO: 23 SEQ ID NO: 24 SEQ ID NO: 25 SEQ ID NO: 26 SEQ ID NO: 27 SEQ ID NO: 4 SEQ ID NO: 28 SEQ ID NO: 29 SEQ ID NO: 30 SEQ ID NO: 32 SEQ ID NO: 31 SEQ ID NO: 32 SEQ ID NO: 33 SEQ ID NO: 34 SEQ ID NO: 35 SEQ ID NO: 36 SEQ ID NO: 37 SEQ ID NO: 38 SEQ ID NO: 39 SEQ ID NO: 40 SEQ ID NO: 41 SEQ ID NO: 42 SEQ ID NO: 43 SEQ ID NO: 44 SEQ ID NO: 45 SEQ ID NO: 46 SEQ ID NO: 47 SEQ ID NO: 48 SEQ ID NO: 49 SEQ ID NO: 50 SEQ ID NO: 51 SEQ ID NO: 52 SEQ ID NO: 53 SEQ ID NO: 54 SEQ ID NO: 55 SEQ ID NO: 57 SEQ ID NO: 56 SEQ ID NO: 57 SEQ ID NO: 58 SEQ ID NO: 59 provided that said sequence may be a complementary sequence or a degenerate sequence thereof. (4) A TCR gene comprising the αCDR3 polynucleotide and the βCDR3 polynucleotide in any one of pairs of (3). (5) The TCR gene of (4) obtainable from a CD4⁺ T-cell specific to WT1₃₃₂ peptide. (6) A method for producing a CD4⁺ helper cell specific to WT1₃₃₂ peptide, comprising introducing the TCR gene of (4) into a CD4⁺ cell. (7) A CD4⁺ helper T-cell obtainable by the method of (5). (8) A vector comprising a TCR gene which comprises the αCDR3 polynucleotide and the βCDR3 polynucleotide in any one of pairs of (3). (9) The method of (6) wherein said introduction is performed using the vector of (8). (10) A method for enhancing the induction of a WT1 specific CTL, comprising co-culturing the CD4⁺ helper T-cell of (7) and a peripheral mononuclear cell. (11) A WT1-specific CTL obtainable by the method of (10). (12) A method for the treatment or prevention of a cancer in a subject, comprising introducing the CD4⁺ helper T-cell of (7) into the subject. (13) A pharmaceutical composition for the treatment or prevention of a cancer, comprising the CD4⁺ helper T-cell of (7). (14) Use of the CD4⁺ helper T-cell of (7) for the manufacture of a medicine for the treatment or prevention of a cancer. (15) A DNA chip comprising the αCDR3 polynucleotide of (1), the βCDR3 polynucleotide of (2), or both of the αCDR3 polynucleotide of (1) and the βCDR3 polynucleotide of (2). (16) A method for measuring the frequency of CD4⁺ helper T-cell specific to WT1₃₃₂ peptide in a sample, comprising using the DNA chip of (15). (17) An αCDR3 peptide encoded by any one of the αCDR3 polynucleotides of (1). (18) A βCDR3 peptide encoded by any one of the βCDR3 polynucleotides of (2). (19) A pair of peptides encoded by any one of pairs of the polynucleotides of (3). (20) A chip comprising the peptide of (17) or (18), or the pair of the peptides of (19). (21) An antibody against any one of the peptides of any one of (17)-(19). (22) A method for measuring the frequency of CD4⁺ helper T-cell specific to WT1₃₃₂ peptide in a sample, comprising using the antibody of (21).

Effect of the Invention

According to the present invention, a CD4⁺ helper T-cell is obtained into which a TCR gene having the CDR3 nucleotide sequence determined by the present invention has been introduced. A. WT1-specific CTL can be induced using said CD4⁺ helper T-cell, and a cancer can be treated or prevented effectively. Further, a DNA chip is prepared using the TCR sequences, and frequency of WT1₃₃₂-specific CD4⁺ helper T-cells in a sample can be measured.

BRIEF DESCRIPTION OF DRAWINGS

FIG. 1A shows nucleotide sequences of CDR3 α-chains and β-chains of TCR of CD4⁺ helper T-cells obtained by the present invention, and amino acid sequences of CDR3 encoded thereby. Number in parentheses positioned at the right end of each sequence presents SEQ ID NOs in SEQUENCE LISTING. V-GENE, J-GENE and J-GENE describe V region, J region and D region in individual genes, respectively.

FIG. 1B shows nucleotide sequences of CDR3 α-chains and β-chains of TCR of CD4⁺ helper T-cells obtained by the present invention, and amino acid sequences of CDR3 encoded thereby. Number in parentheses positioned at the right end of each sequence presents SEQ ID NOs in SEQUENCE LISTING, V-GENE, J-GENE and J-GENE describe V region, J region and region in individual genes, respectively.

FIG. 2A shows interferon-γ production by WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes shown in Table 3 have been introduced.

FIG. 2B shows IL-2 production by WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes shown in Table 3 have been introduced.

FIG. 2C shows TNF-α production response of WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced, to WT1₃₃₂ peptide concentration.

FIG. 2D shows proliferation ability of WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced, in systems into which several kinds of substances are added. WT1₃₃₂ represents the culture in the presence of WT1₃₃₂ peptide α-DP represents the culture in the presence of an anti-HLA-DP antibody. α-DQ represents the culture in the presence of an anti-HLA-DQ antibody, α-DR represents the culture in the presence of an anti-HLA-DR antibody. HLA class I represents the culture in the presence of an anti-HLA class I antibody. HIV represents the culture in the presence of HIV peptide (FRKQNPDIVIYQYMDDLYVG)(SEQ ID NO: 124).

FIG. 2E shows proliferation of WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced, in the presence of PBMC pulsed with several kinds of substances. WT1₃₃₂ represents the stimulation by autologous PBMC pulsed with WT1₃₃₂ peptide. HWT1 represents the stimulation by autologous PBMC pulsed with full length of WT1 protein. HWT3 represents the stimulation by autologous PBMC pulsed with truncated WT1 protein (not containing WT1₃₃₂ sequence). PHA-blast represents the stimulation by PBMC pulsed with PHA-blast lysate. TF1 represents the stimulation by PBMC pulsed with a lysate of leukemic cell line TF-1 expressing WT1. K562 represents the stimulation by PBMC pulsed with a lysate of leukemic cell line K562 expressing WT1.

FIG. 2F shows IFN-γ production by WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced, in the presence of PBMC pulsed with several kinds of substances, WT1₃₃₂ represents the stimulation by autologous PBMC pulsed with WT1₃₃₂ peptide. HWT1 represents the stimulation by autologous PBMC pulsed with full length of WT1 protein. HWT3 represents the stimulation by autologous PBMC pulsed with truncated WT1 protein (not containing WT1₃₃₂ sequence). PHA-blast represents the stimulation by PBMC pulsed with PHA-blast lysate, TF1 represents the stimulation by PBMC pulsed with a lysate of leukemic cell line TF-1 expressing WT1. K562 represents the stimulation by PBMC pulsed with a lysate of leukemic nein line K562 expressing WT1.

FIG. 2G shows the average of the production of several kinds of cytokines in response to WT1₃₃₂ peptide by WT1₃₃₂-specific CD4⁺ helper T-cell lines from three healthy subjects (HLA-DPB1*05:01-positive) into which TCR genes have been introduced. Black bars represent with the stimulation by WT1₃₃₂ peptide. White bars represent without the stimulation.

FIG. 3A shows the frequency of CD3⁺CD8⁺T cells in case PBMC and WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced are co-cultured at the ratio as shown in the figure.

FIG. 3B shows the frequency of the modified WT1₂₃₅/HLA-A*24:02 tetramer-positive CD8⁺T cells in case PBMC and WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced are co-cultured at the ratio as shown in the figure.

FIG. 3C shows the cell number of WT1 specific. CTL in case PBMC and WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced are co-cultured at the ratio as shown in the figure.

FIG. 3D shows the frequency of CD8⁺T cells expressing interferon-γ in response to the stimulation by the modified WT1₂₃₅ in case PBMC and WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced are co-cultured at the ratio as shown in the figure.

FIG. 4A shows the damage as the lysis (%) of HLA-DPB1*05:01-positive leukemic cell line TF-1 expressing WT1 and HLA-DRB1*05:01-negative leukemic cell line TF-1 expressing WT1 by WT1₃₃₂ specific CD4⁺ helper T-cells into which TCR genes have been introduced at the E:T ratio as shown in the figure.

FIG. 4B shows the damage as the lysis (%) of HLA-DPB1*05:01-positive B-LCL cells which have been enforced to express WT1 and HLA-DPB1*05:01-positive B-LCL cells which do not express WT1 by WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced at the E:T ratio as shown in the figure.

FIG. 4C shows the damage as lysis (%) of K562 cell line and HLA-DPB1*05:01-positive leukemic cell line C2F8 expressing WT1 by WT1₃₃₂-specific CDC helper T-cells into which TCR genes have been introduced at the E:T ratio as shown in the figure.

FIG. 4D shows the results by flow-cytometry for the expression of GranzymeB (left) and Perfolin (right) in WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced.

FIG. 4E shows the results by flow-cytometry for the frequency of CD107a producing cells and IFN-γ producing cells of WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR acnes have been introduced, cultured according to the method described in Example 4.

FIG. 4F is a bar graph showing the results for the comparison of the cell damaging activity of WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced against HLA-CPB1*05:01-positive TF-1 cells pretreated with Ac-IETD-Cho, with the cell damaging activity of WT1₃₃₂-specific CD4⁺ helper T-cells into which TCR genes have been introduced against TF-1 cells pretreated with DMSO. Height of bars represents the average value with bars of standard deviation. Asterisk represents p<0.05.

FIG. 5 shows survival curves showing anti-tumor activity in NOG (Registered Trade Mark) mice by human CD4⁺ T-cells into which TCR genes from WT1₃₃₂ specific CD4⁺ T-cells have been introduced. The solid line represents the survival curve of mice into which human CD4⁺ T-cells have been transferred, into which HLA-DPB1*05:01 restricted WT1₃₃₂-specific TCR have been introduced. The broken line represents the survival curve of mice into which human CD4⁺ T-cells have been transferred, into which a control vector have been introduced.

DESCRIPTION OF EMBODIMENTS

The present invention is based on the determination of the polynucleotides encoding α-chain containing CDR3 (hereinafter referred as “αCDR3 polynucleotide”) and the polynucleotides encoding β-chain containing CDR3 (hereinafter referred as “βCDR3 polynucleotide”) of TCR of CD4⁺ helper T-cell clones specific to a WT1 helper peptide. Thus, in one aspect, the present invention provides αCDR3 polynucleotides having nucleotide sequences shown in FIG. 1 (nucleotide sequences selected from the group consisting of SEQ ID NOs: 1, 3, 5, 8, 10, 11, 13, 14, 16, 18, 20, 22, 23, 25, 27, 28, 30, 31, 33, 35, 37, 39, 41, 43, 45, 47, 49, 51, 53, 55, 56, 58), and βCDR3 polynucleotides having nucleotide sequences shown in FIG. 1 (nucleotide sequences selected from the group consisting of SEQ ID NOs: 2, 4, 6, 7, 9, 12, 15, 17, 19, 21, 24, 26, 29, 32, 34, 36, 38, 40, 42, 44, 46, 48, 50, 52, 54, 57, 59).

Preferably, from the viewpoint of expression of receptor function, an αCDR3 polynucleotide and a βCDR3 polynucleotide contained in each clone are contained in one TCR. That is, it is preferable that an αCDR3 polynucleotide and a βCDR3 polynucleotide corresponding to each clone form a pair as shown in FIG. 1. Therefore, in a further aspect, the present invention provides a pair of a αCDR3 polynucleotide and a βCDR3 polynucleotide, wherein each polynucleotide constituting the pair has a nucleotide sequence shown in FIG. 1. Combination of a αCDR3 polynucleotide and a βCDR3 polynucleotide differs according to each clone. The nucleotide sequence of a pair of an αCDR3 polynucleotide and a βCDR3 polynucleotide in each clone are as shown in FIG. 1.

A polynucleotide having a nucleotide sequence complementary to a αCDR3 polynucleotide or a βCDR3 polynucleotide is also included in a αCDR3 polynucleotide or a βCDR3 polynucleotide in addition, a degenerate sequence of a αCDR3 polynucleotide a βCDR3 polynucleotide is also included in a αCDR3 polynucleotide or a βCDR3 polynucleotide so long as it encodes the peptide shown in FIG. 1.

A polynucleotide having a nucleotide sequence identity of 70% or more, for example 75% or more, 80% or more, 85% or more, or 90% or more, for example 92% or more, 94% or more, 96% or more, or 98% or more, to that of a αCDR3 polynucleotide, is also included in a αCDR3 polynucleotide. A polynucleotide having a nucleotide sequence identity of 70% or more, for example 75% or more, 80% or more, 85% or more, or 90% or more, for example 92% or more, 94% or more, 96% or more, or 98% or more, to that of a βCDR3 polynucleotide, is also included in a βCDR3 polynucleotide.

A polynucleotide having a nucleotide sequence hybridizing to a nucleotide sequence of a αCDR3 polynucleotide under a stringent condition is also included in a αCDR3 polynucleotide. A polynucleotide having a nucleotide sequence hybridizing to a nucleotide sequence of a βCDR3 polynucleotide under a stringent condition is also included in a βCDR3 polynucleotide.

Examples of stringent hybridization conditions include a condition where hybridization is performed in a solution containing 5×SSC, 7% (w/v) SDS, 100 μg/ml denatured salmon sperm DNA and 5×Denhardt' solution at 48-52° C., and then washing is performed in 0.1×SSC, 0.5×SSC, 1×SSC or 2×SSC or a condition where hybridization is performed in a solution containing 250 mM NaCl, 25 mN trisodium citrate, 1% SDS, 50% formamide and 200 μg/ml denatured salmon sperm DNA at 42° C., and then washing is performed in solution containing 15 mN NaCl, 1.5 mM trisodium citrate and 0.1% SDS.

In another aspect, the present invention provides peptides encoded by αCDR3 polynucleotides and βCDR3 polynucleotides (referred as “αCDR3 peptide” and “βCDR3 peptide”, respectively). These peptides have the amino acid sequences shown in FIG. 1. Preferably, these peptides form a pair of a αCDR3 peptide and a βCDR3 peptide corresponding to each clone as shown in FIG. 1.

In the present specification, an amino acid sequence of a peptide is expressed by conventional one-letter system or three-letter system.

A peptide encoded by variants of a αCDR3 polynucleotide or a βCDR3 polynucleotide is also included in αCDR3 peptide or βCDR3 peptide. A peptide having an amino acid sequence identity of 70% or more, for example 75% or more, 80% or more, 85% or more, or 90% or more, for example 92% or more, or 94% or more, to that of a αCDR3 peptide, is also included in a αCDR3 peptide. A peptide having an amino acid sequence identity of 70% or more, for example 75% or more, 80% or more, 85% or more, or 90% or more, for example 92% or more, or 94% or more, to that of a βCDR3 peptide, is also included in a βCDR3 peptide. In addition, a peptide having an amino acid sequence of a αCDR3 peptide in which one to several (for example, one, two, three, four or five) amino acids are substituted, deleted or added is also included in a αCDR3 peptide; and a peptide having an amino acid sequence of a βCDR3 peptide in which one to several (for example, one, two, three, four or five) amino acids are substituted, deleted or added is also included in a βCDR3 peptide. It is noted that these variant peptides has similar properties to those of the original αCDR3 peptides or βCDR3 peptides.

These polynucleotides and polypeptides can be prepared using chemical methods and/or biological methods well-known in the art.

In the present invention, the WT1 helper peptide is a peptide having an amino acid sequence shown in SEQ ID NO: 123 (Lys Arg Tyr Phe Lys Leu Ser His Leu Gln Met His Ser Arg Lys His) or a variant amino acid sequence thereof (These peptides are referred as “WT1₃₃₂ peptide”). WT1₃₃₂ peptide may have a partial sequence or a variant sequence of WT1 polypeptide. A peptide consisting of an amino acid sequence shown in SEQ ID NO: 123 or a variant sequence thereof is an example of such a peptide.

It is known that WT1₃₃₂ peptide has an ability to hind to a HLA-DPB1*15:01 molecule, HLA-DPB1*09:01 molecule, HLA-DPB1*05:01 molecule, HLA-DRB1*04:05 molecule or a HLA-DRB1*15:02 molecule.

A variant sequence of the amino acid sequence shown in SEQ ID NO: 123 as above mentioned refers to an amino acid sequence shown in SEQ ID NO: 123 in which one to several (for example, one, two, three, four or five) amino acids are substituted, deleted or added. Or, a variant sequence of the amino acid sequence shown in SEQ ID NO: 123 as above mentioned refers to an amino acid sequence having an identity of 70% or more, for example 75% or more, 80% or more, 85% or more, or 90% or more, to the amino acid sequence shown in SEQ ID NO: 123. Preferably, a peptide having the amino acid sequence shown in SEQ ID NO: 123 or a variant sequence thereof has a length of 25 amino acids or less. A peptide having a variant sequence of the amino acid sequence shown in SEQ ID NO: 123 has similar properties to those of the peptide having the amino acid sequence shown in SEQ ID NO: 123.

In a further aspect, the present invention relates to a TCR gene containing a αCDR3 polynucleotide and a βCDR3 polynucleotide belonging to any pair shown in FIG. 1. Such a TCR gene may be isolated from a CD4⁺ T-cell specific to WT1₃₃₂ peptide, or may be prepared using well-known genetic engineering technology.

In a further aspect, the present invention relates to a CD4⁺ helper T-cell (referred as “TCR gene introduced CD4⁺ helper T-cell”) obtained by introducing a TCR gene containing a αCDR3 polynucleotide and a βCDR3 polynucleotide belonging to any pair shown in FIG. 1 into a CD4⁺ T-cell. A TCR, gene introduced CD4⁺ helper T-cell shows WT1₃₃₂-specific and HLA class II-restricted proliferation and cytokine production.

A skilled person in the art can easily introduce a TCR gene containing a αCDR3 polynucleotide and a βCDR3 polynucleotide belonging to any one of pairs shown in FIG. 1 into a CD4⁺ T-cell. For example, the introduction of a TCR gene can be done using various kinds of vectors, electroporation, or a gene gun, etc. A TCP gene to be introduced can be modified for the purpose such as improvement of TCR expression efficiency.

Therefore, in a further aspect, the resent invention provides a vector containing a TCR gene containing a αCDR3 polynucleotide and a βCDR3 polynucleotide belonging to any pair shown in FIG. 1.

Introduction of a TCR gene may be done by inserting a α-chain gene containing a αCDR3 polynucleotide and β-chain gene containing a βCDR3 polynucleotide into individual vectors, and introducing these vectors into a CD4⁺ T-cell.

Examples of CD4⁺ T-cells into which a TCR gene containing a αCDR3 polynucleotide and a βCDR3 polynucleotide is introduced include CD4⁺ T-cells derived from a HLA-DRB1*15:01-positive subject, a HLA-DPB1*09:01-positive subject, a HLA-DPB1*05:01-positive subject, a HLA-DRB1*04:05-positive subject or a HLA-DRB1*1502-positive subject, but not limited to them. In addition, CD4⁺ T-cells may be derived from a subject having a cancer, may be derived from a subject having no cancer (a healthy subject), or may be derived from a donor for bone marrow transplantation.

In further aspect, the present invention also relates to a WT1₃₃₂-specific CD4⁺ helper T-cell comprising a TCR gene containing a αCDR3 polynucleotide and a βCDR3 polynucleotide belonging to any pair shown in FIG. 1.

Induction of a WT1-specific CTL can be enhanced using a TCR gene-introduced CD4⁺ helper T-cell. Particularly, induction of WT1-specific CTL can be enhanced by co-culturing a TCR gene-introduced CD4⁺ helper T-cell and a peripheral mononuclear cell. Therefore, in further aspect, the present invention provides a method for enhancing the induction of a WT1-specific CTL, comprising co-culturing a TCR gene-introduced CD4⁺ helper T-cell and a peripheral mononuclear cell. In another aspect, the present invention relates to a WT1-specific CTL obtainable by said method.

Methods and conditions for co-culturing a TCR gene-introduced CD4⁺ helper T-cell and a peripheral mononuclear cell are well known in the art. Such methods can be performed either in vivo or in vitro. One kind of a TCR gene-introduced CD4⁺ helper T-cell may be used for enhancing the induction of a WT1-specific CTL. However, preferably two or more kinds of TCR gene-introduced CD4⁺ helper T-cells are used.

Examples of peripheral mononuclear cells used in the method for enhancing the induction of WT1-specific CTLs of the present invention include peripheral mononuclear cells derived from a HLA-DRB1*15:01-positive subject, a HLA-DPB1*09:01-positive subject, HLA-DPB1*05:01-positive subject, a HLA-DRB1*04:05-positive subject or a HLA-DRB1*15:02-positive subject but not, limited to them. Preferably, the peripheral mononuclear cells and the CD4⁺ T-cells are those which have been obtained from a subject in which a cancer should be treated or prevented.

In the co-cultivation, it is preferable that WT1₃₃₂ peptide and/or other WT1 peptides co-exist. Examples of other WT1 peptides include those which have ability to bind to a HLA-DRB1*15:01 molecule, a HLA-DPB1*09:01 molecule, a HLA-DPB1*05:01 molecule, a HLA-DRB104:05 molecule or a HLA-DRB1*15:02 molecule, but not limited to them.

If necessary, the WT1-specific CTLs obtained by the method mentioned above may be further cultured to make the cell numbers increase, and then administrated to a subject, in order to treat or prevent a cancer in the subject. In such a treatment or prevention of a cancer, it is preferable to co-administrate WT1₃₃₂ peptide and/or other WT1 peptides. By the action of the WT1-specific CTL, CTLs specific to other cancer antigens can also be induced.

A TCR gene-introduced CD4⁺ helper T-cell can damage cancer cells expressing WT1. Therefore, in further aspect, the present invention is a method for the treatment or prevention of a cancer in a subject, comprising introducing a TCR gene-introduced CD4⁺ helper T-cell into the subject.

In further aspect, the present invention provides a pharmaceutical composition comprising a TCR gene-introduced CD4⁺ helper T-cell for the treatment or prevention of a cancer, a use of a TCR gene-introduced CD4⁺ helper T-cell for the manufacture of a medicament for the treatment or prevention of a cancer, and, a use of a TCR gene-introduced CD4⁺ helper T-cell for the treatment or prevention of a cancer.

As used herein, “treatment” of a cancer refers not only to the treatment of a cancer such as the inhibition of progress of a cancer, the reduction of a cancer and the destruction of a cancer, but also to the prevention of recurrence of a cancer.

Examples of subjects in which a cancer is treated or prevented include a HLA-DRB1*15:01-positive subject, a HLA-DPB1*09:01-positive subject, a HLA-DPB1*05:01-positive subject, a HLA-DRB1*04:05-positive subject or a HLA-DRB1*15:02-positive subject, but not limited to them. The above subject is not limited to a cancer patient, and may be a person not having a cancer (including a healthy person), or may be a donor for bone marrow transplantation.

Embodiments of the method for the treatment or prevention, the pharmaceutical composition, and the use as mentioned above are described below. However, the embodiments are not limited to those. First, CD4⁺ T-cells are taken from a peripheral blood of a cancer patient who needs a treatment, and a TCR gene containing a αCDR3 polynucleotide and a βCDR3 polynucleotide is introduced into the CD4⁺ T-cells to obtain TCR gene-introduced CD4⁺ helper T-cells. The TOE mete introduced CD4⁺ helper T-cells thus obtained are administered to the cancer patient. Before the administration, the TCR gene-introduced CD4⁺ helper T-cells can be cultured and proliferated under appropriate conditions to obtain a sufficient number of cells, and then they can be administered to the cancer patient.

Either one kind of TCP gene-introduced CD4⁺ helper T-cell or two or more kind of TCP gene-introduced CD4⁺ helper T-cells may be administered. From the viewpoint of improvement of treatment or prevention effect, it is preferable that two or more kinds of TCR gene-introduced CD4⁺ helper T-cells are administered to a subject.

In case that TCP gene-introduced CD4⁺ helper T-cells are administered to a subject, a physician can appropriately decide conditions such as the number of cells to be administered, the frequency of the administration, the interval of the administration. For example, TCR gene-introduced CD4⁺ helper T-cells may be administered only once, or administered separately several times. Typically, in case of an adult subject, the number of the TCR gene-introduced CD4⁺ helper T-cells per dose is in a range between about 10⁹ and about 10¹¹, but not limited these numbers.

In the treatment or prevention method, the pharmaceutical composition and the use described above, it is preferable that WT1₃₃₂ peptide and/or other WT1 peptides are co-administered. A physician cart appropriately decide amount and frequency of administration of WT1₃₃₂ peptide and/or other WT1 peptides. In addition, other anti-cancer therapies or preventions may be combined.

The method for the treatment or prevention, the pharmaceutical composition, and the use described above can be applied to various kinds of cancers, but not limited to, for example, hematologic malignancies, such as acute myelocytic leukemia, acute lymphocytic leukemia, malignant lymphoma, multiple myeloma, chronic myelocytic leukemia, myelodysplastic syndrome, and recurrence after the hematopoietic stem cell transplantation of the same type; solid cancers, such as tongue cancer, gingival cancer, mouth floor cancer, pharyngeal cancer, larynx cancer, salivary gland cancer, and thyroid cancer; thoracic cancers, such as breast cancer, lung cancer, and thymic cancer; gastrointestinal cancers, such as colon cancer, small intestine cancer, gastric cancer, pancreatic cancer, liver cancer, bile duct cancer, gastrointestinal endocrine tumor, and gastrointestinal carcinoid; cancers of urinary and genital tract, such as renal cancer, urothelial cancer, germinoma, Wilms' tumor, prostate cancer, uterine body cancer, cervical cancer, uterine sarcoma, and ovarian malignancy; musculoskeletal malignancies, such as primary malignancy of bone (e.g., osteosarcoma and Ewing's sarcoma) and soft tissue sarcoma; and other cancers, such as skin cancer, neuroblastoma, malignant glioma (glioblastoma), primary malignant lymphoma of the central nervous system, medulloblastoma, and PNET.

The CDR3 regions are the most diverse portions and are the most responsible parts for the specificity of antigen recognition. Thus, the sequences of the αCDR3 polynucleotides, the βCDR3 polynucleotides, the αCDR3 peptides, and the βCDR3 peptides of the present invention are considered peculiar to the CD4⁺ helper T-cells specific to WT1₃₃₂ peptide. Therefore, in case that a polynucleotide encoding a CDR region of a α-chain and a β-chain, or a peptide corresponding to the CDR region have the sequence of the polynucleotide or the peptide of the present invention, the CD4⁺ helper T-cell is considered to be specific to WT1₃₃₂ peptide.

For example, (i) a DNA chip comprising one or more kinds of αCDR3 polynucleotides, (ii) a DNA chip comprising one or more kinds of βCDR3 polynucleotides, or (iii) a DNA chip comprising both one or more kinds of αCDR3 polynucleotides and one or more kinds of βCDR3 polynucleotides can be used to measure the frequency of CD4⁺ helper T-cells specific to WT1₃₃₂ peptide in a sample. Particularly, a sample is prepared by lysing cells in a specimen obtained from a subject and extracting nucleic acids, and the sample is contacted with the DNA chip.

For example, in case that a sample is contacted with the chip (and hybridization is found at any position, the same sample is contacted with the chip (ii) to confirm whether hybridization is found or not. Then, in case that any hybridization in the chip (i) and any hybridization in the chip (ii) occur with any αCDR3 polynucleotide and any βCDR3 polynucleotide which constitute any pair shown in FIG. 1, it can be judged that a CD4⁺ helper T-cell specific to WT1₃₃₂ peptide having a functional TCR exists in the sample. Using the chip (III), the above process can be done in one step.

A DNA chip may be in any form such as a microchip and a microarray. These chips can be prepared by a well-known method. For example, αCDR3 polynucleotides and βCDR3 polynucleotides can be immobilized on a glass substrate by a well-known method. It is preferable that a label which can indicate presence or absence of hybridization and amount of the hybridization is attached to DNAs in a sample or DNA sequences on a chip.

Not only a DNA chip but also techniques such as southern blotting, northern blotting, colony hybridization can be used to measure frequency of CD4⁺ helper T-cells specific to WT1₃₃₂ peptide in a sample.

In addition, a αCDR3 peptide and a βCDR3 peptide can be used to obtain an antibody to a CD4⁺ helper T-cell specific to WT1₃₃₂ peptide. A CD4⁺ helper T-cell specific to WT1₃₃₂ peptide can be detected using such an antibody. A receptor of a CD4⁺ helper T-cell specific to WT1₃₃₂ peptide can also be stimulated using such an antibody. Such stimulation can be done either in vivo or in vitro.

A chip comprising αCDR3 peptides, a chip comprising βCDR3 peptides, or a chip comprising both αCDR3 peptides and βCDR3 peptides can also be used to detect an antibody to a CD4⁺ helper T-cell specific to WT1₃₃₂ peptide.

A chip comprising these peptides can be prepared using a well-known method. It is preferable to add a label which can determine presence or absence of a specific binding to peptides in a sample or peptides on a chip.

A chip comprising antibodies to αCDR3 peptides and/or βCDR3 peptides can also be used to determine kind and amount of βCDR3 peptides and/or βCDR3 peptides in a sample, or to determine kind and amount of CD4⁺ helper T-cells specific to WT1₃₃₂ peptide in a sample.

A chip to which these antibodies are immobilized can be prepared using a well-known method. It is preferable to add a label which can determine presence or absence of a specific binding to peptides in a sample or antibodies on a chip.

Description of Sequences

SEQ ID NOs: 1 to 59 are nucleotide sequences encoding CDR3 contained in TCR of CD4⁺ helper T-cell clones.

SEQ ID NOs: 60 to 118 are amino acid sequences of CDR3 contained in TCR of CD4⁺ helper T-cell clones.

SEQ ID NO: 119 is a reverse primer for amplifying TCRα chain.

SEQ TD NO: 120 is a reverse primer for amplifying TCRβ chain.

SEQ ID NO: 121 is a reverse primer for amplifying TCRβ chain.

SEQ ID NO: 122 is a primer for determining CDR3 nucleotide sequences.

SEQ ID NO: 123 is an amino acid sequence of WT1₃₃₂ peptide,

SEQ ID NO: 124 is an amino acid sequence of HIV peptide.

SEQ ID NO: 125 is an amino acid sequence of a variant of a naturally occurring WT1 peptide.

The present invention is described more particularly and more concretely by showing examples below. However, it should not be construed that examples limit the scope of the present invention.

Example 1

Example 1 Establishment of WT1₃₃₂-specific CD4⁺ T-cell clones and isolation and sequencing of T-cell receptor (TCR) genes

The experimental procedures were as follows.

(1) Method of establishing WT1₃₃₂-specific CD4⁺ T-cell clones

(i) Peripheral blood mononuclear cells (PBMCs) derived from a healthy subject are harvested and seeded into 24-well plates at 3×106 cells/well. X-VIVO 15 medium supplemented with 10% AB serum and 40 IU/ml IL-2 is used as a medium.

(ii) WT1₃₃₂ peptide is added to the above i at a final concentration of 20 μg/ml and the cells are cultured for 7 days.

(iii) After 7 days, the cells are collected and prepared with X-VIVO 15 medium supplemented with 10% AB serum so that the cell density is 1×107 cells/mi, and then, seeded by 100 μL each into 96 well, round bottom plates.

(iv) WT1₃₃₂ peptide, BD GolgiStop™ (BD Bioscience) and CD28/CD49d Costimulatory Reagent (BD Bioscience) are added to X-VIVO 15 medium supplemented with 10% AB serum at final concentrations of 40 μg/ml, 4 μg/ml, and 4 μg/ml, respectively.

(v) The above iv is added by 100 μL each to the above iii.

(vi) Anti-human C154-APC-labeled antibody (BD Bioscience) is added by 10 μl each to the above v and the plates are incubated in 5% CO₂ incubator for 6 hours at 37° C.

(vii) After incubation, the cells are collected and stained with anti-human CD4-APC-H7-labeled antibody (BD Bioscience) and anti-human CD3-Pacific Blue-labeled antibody (BD Bioscience) as well as 7-AAD (eBioscience) for removing dead cells.

(viii) PBMCs are harvested from 3 healthy subjects, mixed, irradiated with 30 Gy of γ-ray, and prepared with X-VIVO 15 medium supplemented with 10% AB serum at a final concentration of 10%, IL-2 at a final concentration of 100 IU/ml, and PHA at a final concentration of 3 μg/ml so that the cell density is 1×106 cells/ml. These prepared cells are seeded by 100 μL each into 96 well, round bottom plates.

(ix) 7-ADD-CD3⁺CD4⁺CD154⁺ cell fraction, i.e., a fraction containing WT1₃₃₂-specific CD4⁺ T-cells is single-cell sorted into each well of the above viii using FACSAria cell sorter.

(x) After culture for 10-14 days, the proliferated cells in each well are used as independent CD4⁺ T-cell clones.

(2) Screening of WT1₃₃₂-specific CD4⁺ T-cell clones

(i) Each CD4⁺ T-cell clone of the above (1)-x is prepared with X-VIVO 15 medium supplemented with 1% AB serum so that the cell density is 3×105 cells/ml.

(ii) Autologous PBMCs pulsed with WT1₃₃₂ or not pulsed with any peptides are irradiated with 30 Gy of γ-ray and prepared with X-VIVO 15 medium supplemented with 1% AB serum so that the cell density is 1×106 cells/ml.

(iii) The above (2)-i and ii are seeded by 100 μL each into 96 well, round bottom plates.

(iv) After culture for 2 days, 3H-thymidine is added to each well at 1 μCi/well.

(v) After 18 hours, the 3H-thymidine incorporated into each CD4⁺ T-cell clone is measured and the CD4⁺ T-cell clones showing WT1₃₃₂

specific proliferative response are selected. These selected clones are used as WT1₃₃₂-specific CD4⁺ T-cell clones.

(vi) The culture of the WT1₃₃₂ specific CD4⁺ T-cell clones is performed with stimulation of the WT1₃₃₂ specific CD4⁺ T-cell clones by co-culturing with PBMCs that were prepared by irradiating autologous PBMCs pulsed with WT1₃₃₂ at a frequency of once per 1-2 weeks or so with 30 Gy of γ-ray.

(3) Isolation of TCR genes using 5′-RACE (Rapid Amplification of cDNA End) method

(i) WT1₃₃₂-specific CD4⁺ T-cell clones are cultured for 10 days or more from the last stimulation. This is to prevent contamination with T-cells contained in autologous PBMCs that are used for the stimulation.

(ii) The WT1₃₃₂-specific CD4⁺ T-cell clones are pelleted, TRIzol reagent (Invitrogen) is added thereto, and RNA is extracted according to its manual.

(iii) cDNAs are synthesized from the RNA extracted in the above (3)-ii using SMARTer™ RACE cDNA Amplification Kit (Clontech).

(iv) TCR α-chain and β-chain genes are amplified by using the cDNAs synthesized in the above (3)-iii as templates. In regard to used primers, UPM primer included in MARTer™ RACE cDNA Amplification Kit was used as a forward primer and the following TCR-specific primers were used as reverse primers:

Cα3′UTR-primer: (SEQ ID No: 119) 5′-CAC AGG CTG TCT TAC AAT CTT GCA GAT C-3′ Cβ1-3′UTR-primer: (SEQ ID No: 120) 5′-CTC CAC TTC CAG GGC TGC CTT CA-3′ Cβ2-3′UTR-primer: (SEQ ID No: 121) 5′-TGA CCT GGG ATG GTT TTG GAG CTA-3′.

(v) The amplification of the TCR genes was performed using KOD FX available from ToYoBo under conditions of 94° C., 3 min→(98° C., 10 sec→68° C., 1 min)×35 cycles.

(vi) The size of PCR products are confirmed using agarose gel electrophoresis and bands of near 1 kbp are cut from gel and purified.

(vii) After adenines are added to the PCR products purified in the above (3)-vi using Taq polymerase, the resultants are ligated into pCR 2.1 vectors.

(viii) HST02 competent cells are transformed with the above (3)-vii, plasmids are purified from single colonies, and then, sequenced.

(ix) The sequence analysis is performed using the International Immunogenetics Information System and each TCR gene is identified.

With regard to the above (3) “isolation of TCR genes using 5′-RACE (Rapid Amplification of cDNA End) method”, the detailed experimental procedure is shown below.

(3-1) RNA Extraction

RNA extraction from T-cell clones was performed using TRIzol Reagent (Invitrogen). As for T-cell clones used, the clones cultured without antigen-stimulation art the presence of IL-2 over 3 weeks were prepared for the purpose of preventing contamination with feeder cells.

(3-2) Cloning of full-length TCR (T-cell receptor) cDNA using 5′-RACE (Rapid Amplification of cDNA Ends) method

For cloning of TCR α/β, SMARTer™ RACE cDNA Amplification Kit (Clontech) was used. Firstly, 5′-RACE reaction was performed according to its manual, and thereby 1st strand cDNA was synthesized. Then, in order to obtain ti full-length TCR α-chain and β-chain cDNAs, PCR reaction was performed by using reverse primers specific to each of 3′UTRs (Untranslated Regions) and, universal primer (UPM) which is included in the kit and using the synthesized 1st strand cDNA as a template. The used primers are as follows.

Cα 3′UTR-RACE-primer: (SEQ ID No: 119) CACAGGCTGTCTTACAATCTTGCAGATC Cβ1 3′UTR-RACE-primer: (SEQ ID No: 120) CTCCACTTCCAGGGCTGCCTTCA Cβ2 3′UTR-RACE-primer: (SEQ ID No: 121) TGACCTGGGATGGTTTTGGAGCTA

Further, FOR reaction was performed in the following reaction solution composition using KOD FX (TOYOBO).

TABLE 1 2x PCR buffer for KOD FX 12.5 μl 2 mM dNTPs 5.0 μl 10x UPM 2.5 μl 10 μM reverse primer 1.0 μl Template DNA 1.0 μl KOD FX (1.0 U/μl) 0.5 μl distilled water up to 25 μl Volume of the reaction solution 25 μl PCR cycle is as follows: 94° C., 2 min −> (98° C., 10 sec −> 68° C., 1 min) × 35 cycles −> 15° C., hold

After the PCR reaction, 1.0% agarose gel electrophoresis was performed, single bands of near 900-1000 bp were cut, and the PCR products were purified with 50 μl of distilled water using QTAquick Gel Extraction Kit (QIAGEN). It is necessary to add adenine to both ends of the PCR products for TA-cloning. The addition of adenine was performed using Platinum Tag DNA polymerase (invitrogen) as follows.

(1) 2× reaction solution shown in the table below is prepared.

TABLE 2 10x PCR buffer 10 μl 2 mM dNTPs 10 μl 25 mM MgCl2 8.0 μl Platinum Taq polymerase 1.0 μl 21 μl of distilled water is added so that a total volume is 50 μl.

(2) 2× reaction solution is incubated at 95° C. for 5 minutes.

(3) The purified PCR products are added thereto.

(4) The resultants are incubated at 72° C. for 10 minutes.

PCR products added with adenines were purified and concentrated by ethanol precipitation, and then, inserted into pCR 2.1 vectors (invitrogen) using DNA Ligation Kit, Mighty Mix>(TaKaRa). pCR 2.1 vectors comprising the POP products were introduced into HST02 competent cells by transformation and cloned.

(3-3) Purification of plasmids comprising full-length TCR α-chain and β-chain cDNAs

The transformed HST02 competent cells were plated on ampicillin/LB plates and incubated at 37° C. Then, single colonies were picked into ampicillin/LB liquid medium, and incubated 37° C. while being stirred at 200 rpm. Then, plasmids were purified from the Escherichia coli solution using AUTOMATIC DNA ISOLATION SYSTEM PI-50 (KURABO).

(3-4) Determination of CDR3 sequence of TCR by sequencing

For sequencing of the purified plasmids, BigDye® Terminator v3.1 Cycle Sequencing Kit (Applied Biosystems) was used. In addition, M13 reverse primer:

(SEQ ID No: 122) caggaaacagctatgac was used. For analysis of TCR and CD3, IMGT/V-QUEST was utilized.

The determined nucleotide and amino acid sequences of CDR3 are shown in FIG. 1. In some of the clones, there were 2 kinds of α-chain and 2 kinds of CDR 3 sequences.

Example 2

Example 2 introduction of T-cell receptor (TCR) genes derived from a WT1₃₃₂-specific CD4⁺ T-cell to human CD4⁺ T-cells

It was confirmed that human CD4⁺ T-cell transduced with T-cell receptor (TCR) genes derived from a WT1₃₃₂-specific CD4⁺ T-cell showed proliferative response and production of cytokines in a WT1₃₃₂-specific and HLA class II-restricted manner.

TCR genes shown in Table 3 were isolated from clone 9 which is the CD4⁺ T-cell clone which specifically recognizes WT1₃₃₂ in an HLA-DPB1*05:01-restricted manner. These TCR genes were transduced into CD4⁺ T-cells derived from peripheral blood of healthy subjects by using lentivirus vectors, and the response to WT1₃₃₂ was examined by using the productions of cytokines (interferon-γ and IL-2) as indicators (FIGS. 2A and B). In addition, CD4⁺ T-cells transduced with lentivirus vectors not carrying TCR genes (indicated as mock) were used as a control, CD4⁺ T-cells transduced with WT1₃₃₂-specific TCR genes (referred as “WT1₃₃₂-TCR-transduced CD4⁺ T-cells” in the section or Examples) produced INF-γ and IL-2 in response only to WT1₃₃₂, i.e., in a WT1₃₃₂-specific manner. On the other hand, the mock-transduced CD4⁺ T-cells did not show WT1₃₃₂-specific production of cytokines.

The effect of the concentration of WT1₃₃₂ peptide on the expression of cytokine by WT1₃₃₂-TCR-transduced CD4⁺ T-cells was examined, WT1₃₃₂-TCR-transduced CD4⁺ T-cells were stimulated with various concentrations of WT1₃₃₂ peptide for 4 hours, and intracellular cytokine staining assay was performed to examine the ratio of TNF-α-producing CD4⁺ T-cells to CD4⁺ T-cells. The results are shown in FIG. 2C. The production of the cytokine was WT1₃₃₂ peptide concentration-dependent and ED50 was 4.85 μM.

When a proliferation potency of the WT1₃₃₂-TCR-transduced CD4⁺ T-cells was examined, a WT1₃₃₂-specific, strong proliferation potency was found and the proliferative response was markedly inhibited by anti-HLA-DP antibody (FIG. 2D).

Next, the proliferative response and IFN-γ production of the WT1₃₃₂ TCR-transduced CD4⁺ T-cells to autologous PBMCs pulsed with WT1₃₃₂ peptide, autologous PBMCs pulsed with full-length WT1 protein, autologous PBMCs pulsed with truncated. WT1 protein (not comprising WT1₃₃₂ sequence), PBMCs pulsed with the lysate of PHA-blast, PBMCs pulsed with the lysate of leukemia cell line TF-1 expressing WT1, and PBMCs pulsed with the lysate of leukemia cell line K562 expressing WT1 were examined. The cell proliferation was measured by [3H]-thymidine incorporation, and IFN-γ was measured by ELISA. The results are shown in FIG. 2E and FIG. 2F, respectively. It was found that the proliferation and IFN-γ production of the WT1₃₃₂ TCR-transduced CD4⁺ T-cells were markedly stimulated by PBMCs pulsed with the lysate of leukemia cell lines (TF-1 and K562) expressing WT1 and also stimulated by autologous PBMCs pulsed with WT1₃₃₂ peptide and autologous PBMCs pulsed with full-length WT1 protein.

Further, the production of various cytokines that responded to WT1₃₃₂ peptides of WT1₃₃₂-TCR-transduced CD4⁺ T-cell lines prepared similarly to those of Example 2, that were derived from 3 healthy (HLA-DPB1*05:01 positive) donors (i.e., three kinds of cell lines), was also examined. The mean values of the cytokine-producing abilities of the three kinds of cell lines are shown in FIG. 2G. Th1-type cytokines such as IL-2, IFN-γ, TNF-α and GM-CSF were produced in large amount.

TABLE 3 TCR genes isolated form clone 9 V gene J segment D gene CDR3 sequence Va TRAV13- TRAJ53* — CAENSGGSNYKLTF 8.2 2*01 01 (SEQ ID No: 73) Vb TRAB6- TRBJ1- TRBD01* CASTAGASDQPQHF  13.3 1*01 5*01 01 (SEQ ID No: 74)

Example 3

Example 3 Enhanced induction of WT1-specific CTLs by human CD4⁺ T-cells transduced with TCR genes derived from WT1₃₃₂-specific CD4⁺ T-cells

Generally, it is known that CD4⁺ T-cell serves as helper T-cell and is important for introduction and maintenance of CD8⁺ T-cells (CTLs) that are the primary effector cells that attack cancer cells. Thus, it was examined whether WT1₃₃₂-TCR-transduced CD4⁺ T-cells enhanced the induction of WT1-specific CTLs.

PBMCs of HLA-A*24:02 and HLA-DPB1*05:01-positive healthy subjects were mixed with WT1₃₃₂-TCR-transduced CD4⁺ T-cells prepared from the same healthy subjects at the ratio of 10:1 and 5:1 (indicated as 1:0.1 and 1:0.2 in FIG. 3) and incubated for 1 week in the presence of a modified WT1₂₃₅ peptide (wherein M, the second amino acid of natural WT1 peptide binding to HLA-A*24:02 molecule, was modified into Y (CYTWNQMNL)(SEQ ID No:125)) that is an HLA-A*24:02-restricted CTL epitope derived from WT1 and WT1₃₃₂. Then, the resultant was stimulated again with the modified WT1₂₃₅ peptide (wherein the binding ability to HLA-A*24:02 molecule were enhanced) and further incubated for 1 week. No IL-2 was added in a series of cultures in order to correctly evaluate the help activity of CD4⁺ T-cells. After 2 weeks cultures in total, it was examined whether the induction of WT1-specific CTLs was enhanced by the WT1₃₃₂ TCR-transduced CD4⁺ T-cells by using frequencies of CD8⁺ T-cells, modified WT1/HLA-A*24:02 tetramer-positive CD4⁺ T-cells, and modified WT1₂₃₅-specific interferon-γ (INF-γ)-expressing CD8⁺ T-cells as indicators. As a result, the frequency of CD8⁺ T-cells was significantly higher when co-cultured with the WT1₃₃₂-TCR-transduced CD4⁺ T-cells as compared when cultured with the mock-transduced CD4⁺ T-cells as a control (FIG. 3A). In addition, in regard to the modified WT1₂₃₅/HLA-A*24:02 tetramer positive CD8⁺ T-cells that are el-specific CTLs, a clearly positive population was found when co-cultured with the WT1₃₃₂-TCR-transduced CD4⁺ T-cells, however, it was not found in the control (FIG. 3B). Calculating the cell number of the WT1-specific CTLs present in 100,000 lymphocytes from these results, the cell number was about 28 times higher when co-cultured with the WT1₃₃₂-TCR-transduced CD4⁺ T-cells compared with the control (FIG. 3C). Likewise, the frequency of CD8⁺ T-cells expressing INF-γ by the stimulation with the modified WT1₂₃₅ was also significantly high when co-cultured with the WT1₃₃₂-TCR-transduced CD4⁺ T-cells (FIG. 3D). From the above, it was revealed that the WT1₃₃₂-TCR-transduced CD4⁺ T-cells enhanced the induction of WT1-specific CTLs.

Example 4

Example 4 HLA-DPB1*05:01-restricted damage of WT1-expressing leukemia cells by human CD4⁺ T-cells transduced with TCR genes derived from WT1₃₃₂-specific CD4⁺ T-cells

Next, the cytotoxic activity, i.e., killing activity, of WT1₃₃₂-TCR-transduced CD4⁺ T-cells was evaluated.

Firstly, HLA-DPB1*05:01 gene was isolated and transfected into leukemia cell line TF-1 expressing WT1 to prepare HLA-DPB1*05:01-positive TF-1 cells. As shown in FIG. 4A, the WT1₃₃₂-TCR-transduced CD4⁺ T-cells strongly damaged HLA-DPB1*05:01-positive TF-1 cells, however, they did not exhibit cytotoxic activity on HLA-DPB1*05:01-negative TF-1 cells. Then, in order to confirm whether this cytotoxic activity is WT1-specific, B-LCL(+) was prepared by overexpressing WT1 gene in HLA-DPB1*05:01-positive B-LCL cells not expressing WT1 (indicated as B-LCL(−)), and these cells were used as target cells to evaluate the cytotoxic activity of WT1₃₃₂-TCR-transduced CD4⁺ T-cells. As shown in FIG. 4B, B-LCL(+) was strongly damaged by the WT1₃₃₂-TCR-transduced CD4⁺ T-cells, however, B-LCL(−) was not damaged. From these results, it was revealed that the WT1₃₃₂-TCR-transduced CD4⁺ T-cells had the HLA-DPB1*05:01-restricted and WT1-specific cytotoxic activity. Further, the cytotoxic activity of the WT1₃₃₂-TCR-transduced CD4⁺ T-cells was confirmed by using leukemia cell line C2F8 which was HLA-DPB1*05:01-positive and expressed WT1 (FIG. 4C).

Next, it was examined whether WT1₃₃₂-TCR-transduced CD4⁺ T-cells exerted the cytotoxic activity via the granzyme B and perforin pathway. High expressions of granzyme B and perforin were found in the WT1₃₃₂-TCR-transduced CD4⁺ T-cells (FIG. 4D).

WT1₃₃₂-TCR-transduced CD4⁺ T-cells and CD4⁺ T-cells similarly treated with mock-vector (mock-transduced CD4⁺ T-cells) were cultured with HLA-DPB1*05:01-positive TF-1 cells pulsed with WT1₃₃₂ peptide or HLA-DPB1*05:01-positive TF-1 cells not pulsed with WT1₃₃₂ peptide for 5 hours in the presence of anti-CD107a-APC-monoclonal antibody. Then, IFN-γ-staining was performed and the resultants were subjected to Flow cytometry. The co-expression of IFN-γ and CD107a was found in the WT1₃₃₂-TCR-transduced CD4⁺ T-cells only when the WT1₃₃₂-TCR-transduced CD4⁺ T-cells were incubated with HLA-DPB1*05:01-positive TF-1 cells pulsed with WT1₃₃₂ peptide (FIG. 4E). This shows that the degranulation occurs in the WT1₃₃₂-TCR-transduced CD4⁺ T-cells.

To confirm whether the cytotoxic activity of the WT1₃₃₂-TCR-transduced CD4⁺ T-cells was dependent on the granzyme B/perforin pathway, HLA-DPB1*05:01-positive TF-1 cells pretreated with 100 μM of a granzyme-inhibitor, Ac-IETD-Cho, were used as target cells. The HLA-DPB1*05:01-positive TF-1 cells were pretreated with 100 μM of Ac-IETD-Cho or DMSO (control) for 2 hours, then labeled with ⁵¹Cr, and incubated with WT1₃₃₂-TCR-transduced CD4⁺ T-cells, and ⁵¹Cr releasing assay was performed. The cytotoxic activity of the WT1₃₃₂-TCR-transduced CD4⁺ T-cells on HLA-DRB1*05:01-positive TF-1 cells pretreated with Ac-IETD-Cho was markedly lower compared with the cytotoxic activity on TF-1 cells pretreated with DMSO (FIG. 4F).

Considering these results together, it was confirmed that the WT1₃₃₂-TCR-transduced CD4⁺ T-cells obtained by the present invention directly recognized HLA-DPB1*05:01-positive leukemia cells expressing WT1 and damaged them via granzyme B/perforin pathway.

Example 5

Example 5 Anti-tumor effect in NOG® Mouse by human CD4⁺ T-cells transduced with TCR genes derived from WT1₃₃₂-specific CD4⁺ T-cells

WT1-expressing HLA-DPB1*05:01-positive human leukemia cells C2F8 (5×104 cells) were transferred to NOG® mice (7 mice) via tail vein. Next day, as an experimental group, human CD4⁺ T-cells transduced with HLA-DPB105:01-restricted WT1₃₃₂-specific TCR genes (SEQ ID Nos: 14 and 15) (5×106 cells) and T-cell-depleted human peripheral blood mononuclear cells (2×106 cells) from the same subject as antigen-presenting cells were transferred to the above NOG® mice (3 mice). As a control, human CD4⁺ T-cells transduced with the control vector (5×106 cells) and T-cell-depleted human peripheral blond mononuclear cells (2×106 cells) from the same subject as antigen-presenting cells were transferred to the above NOG® mice (4 mice).

After 1 and 2 weeks, human CD4⁺ T-cells transduced with HLA-DPB1*05:01-restricted WT1₃₃₂-specific TCR genes (5×106 cells) were transferred to the mice of the experimental group via tail vein. Human CD4⁺ T-cells transduced with control vector (5×106 cells) were transferred to the control mice via tail vein. Then, the survival of mice was examined.

The results are shown in FIG. 5. Since the survival rate of the mice of the experimental group exceeded the survival rate of the mice of control, it was shown that HLA-DPB1*05:01-restricted WT1₃₃₂-specific TCR-transduced human CD4⁺ T-cells had an anti-tumor effect in vivo.

INDUSTRIAL APPLICABILITY

The present invention can be used in the fields of pharmaceuticals for treating or preventing cancer, of reagents for cancer research, and of cancer test kits or reagents, and the like. 

The invention claimed is:
 1. A DNA chip comprising (i) a αCDR3 polynucleotide having a nucleotide sequence selected from the group consisting of SEQ ID NOs: 1, 3, 5, 8, 10, 11, 13, 14, 16, 18, 20, 22, 23, 25, 27, 28, 30, 31, 33, 35, 37, 39, 41, 43, 45, 47, 49, 51, 53, 55, 56 and 58, or (ii) a βCDR3 polynucleotide having a nucleotide sequence selected from the group consisting of SEQ ID NOs: 2, 4, 6, 7, 9, 12, 15, 17, 19, 21, 24, 26, 29, 32, 34, 36, 38, 40, 42, 44, 46, 48, 50, 52, 54, 57 and 59, or (iii) both the αCDR3 polynucleotide and the βCDR3 polynucleotide. 